Originally posted by jsun529
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Thank you very much for all your help, since I am very new to this BFAST program, The program runs pretty fast and with the new version it runs pretty smoothly. For my test run on solid, when I use the sam tools to call variants, the result was not what I expected, I think it comes to both side, one is the samtools, another is I think more critical as how to create proper indexes, for snp and indels? Looks like with new version this is the only parameter left to the user? Thanks
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The same parameters are available, they just now default to the recommended settings for whole-genome human resequencing. The indexes are important, and depend on read length, error rates, and polymorphism rate (snp and indel). What read length, error rate, platform, and polymorphism rate are you considering?Originally posted by jsun529 View PostThank you very much for all your help, since I am very new to this BFAST program, The program runs pretty fast and with the new version it runs pretty smoothly. For my test run on solid, when I use the sam tools to call variants, the result was not what I expected, I think it comes to both side, one is the samtools, another is I think more critical as how to create proper indexes, for snp and indels? Looks like with new version this is the only parameter left to the user? Thanks
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Hi Nils,
I found Bfast challenging to get into as well. I saw that as someone who has been using Maq, Mosaik, Bowtie and so on for quite some time now.
There is plenty of detail in the manual but the program expects you to set parameters right from the off, without any suggestion of defaults. Now it may well be this is complicated and reference dependent, but to encourage users I would strongly recommend
a) a short sample reference, say a genomic island or 500k of a genome
b) a few reads which can be mapped onto this.
There is plenty of public data about now.
Then I would have a group of command lines in place of the "quick tutorial" links.
For users unfamiliar with installing from c source instructions could be provided as well.
I m sure potential users would appreciate the effort involved in doing this
Colin
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Great suggestions! What was the last version you used? I say that because an overhaul was made between 0.5.x and 0.6.x to improve the user interface, manual, and set default/recommended parameters.Originally posted by colindaven View PostHi Nils,
I found Bfast challenging to get into as well. I saw that as someone who has been using Maq, Mosaik, Bowtie and so on for quite some time now.
There is plenty of detail in the manual but the program expects you to set parameters right from the off, without any suggestion of defaults. Now it may well be this is complicated and reference dependent, but to encourage users I would strongly recommend
a) a short sample reference, say a genomic island or 500k of a genome
b) a few reads which can be mapped onto this.
There is plenty of public data about now.
Then I would have a group of command lines in place of the "quick tutorial" links.
For users unfamiliar with installing from c source instructions could be provided as well.
I m sure potential users would appreciate the effort involved in doing this
Colin
There is a quick tutorial at the end of the manual giving examples and the recommended parameters (the program now has defaults). Does this address the issue?
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